mapping by pcr
TRANSCRIPT
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MOLECULAR MAPPING
BY PCR-Sapate P D,
ABW/34/2011.
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INTRODUCTION
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POLYMARASE CHAIN
REACTION It is an in vitro amplification of template DNA using
a basic principle of “semi conservative replication of DNA” naturally found in living cell.
It is completely an automated reaction carried out a thermo cycler , utilizes following things-
• Template DNA
• Two oligonucleotide primers
• dNTP’s
• Heat stable DNA polymerase
It generates billion copies of DNA , present even as a single copy in the initial preparation, within few hours.
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PCR involves amplification of a specific gene
or DNA sequence within a very less duration.
Specificity is one of the important attribute
of PCR.
It generally involves following steps-Step Temperature(˚
C)
Duration Description
Denaturation 94 2 min Two strands of DNA
get separated
Primer
annealing
40-60 1 min Primer get joined to 3’
end of any strand
Extension 72 2 min New strand formation
at free 3’end of primer
by taq polymerase
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This is a single cycle for a few minutes.
In thermal cycler, this cycle is automatically
repeated for 30-40 times which requires few
hours to complete.
PCR has wide range of applications, one of is
‘creation of molecular(genome) maps’.
Previously biochemical & protein based
markers used but PCR makes revolutionary
change in this field.
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MOLECULAR MAPS
It may be defined as “a detailed structure &
functional organization of the complete genome of
an organism”.
The ultimate aim is to obtain the DNA sequences
of the complete genome , which provides most
detailed molecular description.
Initially , traits were observable with naked eyes
were used for mapping, then comes isozymes
markers. But due to there lack of availability in the
genome , molecular markers used to produce
genome maps.
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These were divided in following categories-
Genetic mapping:
It is an schematic representation of
various genetic markers in the specific orders
in which they are located in chromosome as
well as the relative distances between these
makers.
The distance is given in terms of
centiMorgan(cM) which are proportionate to
recombination frequencies.
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Physical mapping :
It uses molecular biology techniques to
examine DNA molecules directly in order to
construct maps showing the positions of
sequence features, including genes.
The distance shows actual number of base
pairs present within the two possible genes.
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Genetic map, serves to guide a scientist
toward a gene, just like an interstate map
guides a driver from city to city.
Physical maps mark an estimate of the true
distance, in measurements called base pairs,
therefore, allow a scientist to more easily
home in on the location of a gene.
Both genetic and physical maps provide the
likely order of items along a chromosome.
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Linkage analysis is the basis of
genetic mapping
Chromosomes are inherited as intact units, so it was reasoned that the alleles of some pairs of genes will be inherited together because they are on the same chromosome. This is the principle of ‘genetic linkage’.
Pairs of genes were either inherited independently, as expected for genes in different chromosomes, or, if they showed linkage, then it was only partial linkage: sometimes they were inherited together and sometimes they were not.
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HISTORY
1913- first linkage map was constructed in
drosophila melanogaster.
1985-PCR was developed by kary mullis.
1988- Olson et al suggested STS’s(sequence
tagged sites) for physical mapping of human
genome.
1989-kary mullis discovered thermo stable
polymerase (taq polymerase).
“Science” announced taq polymerase as
‘molecule of the year’.
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1993- Kleinhofs et al constructed first whole
genome linkage maps of barley based on
molecular markers (mainly RFLPs).
2006-A potato linkage map was generated
with over 10,000 AFLP loci by Van Os et al .
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WHY PCR USED IN
MAPPING?
Using gene as a marker is very useful but it has
limitation.
Gene occupy very small portion/space of
genome and are not evenly distributed in the
genome.
Also every gene not have allelic forms or can
not distinguishable easily.
Therefore the map based on gene is not
detailed.
So there comes need of other markers, which
is fulfilled by DNA markers(PCR based
markers).
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DIFFERENT PCR BASED
MARKERS USED FOR MAPPING
A molecular marker is polymorphic DNA sequence used for chromosome mapping.
A marker is said to be polymorphic if it has different forms in different individual of a species.
There were mainly 3 PCR based markers used to prepare genetic maps .
• RAPD
• AFLP
• STS
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RAPD
It is an Random Amplified Polymorphic DNA, which uses random/arbitrary oligonucleotide primers (pronounced as ‘rapids’).
The size of primer used ranges 2 – 10 bp which is not specific.
Genomic DNA has complementary sequences to RAPD primers to many location.
After PCR, in some strains which has complementary region detected in gel but those do not having region can not be detected.
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These bands constitute the ‘RAPD loci’.
RAPD marker is dominant marker i.e.
presence of band is dominant & absence of
band is recessive.
DNA bands of different sizes are assumed to
be amplified product of different RAPD loci in
the genome.
RAPD markers shows limited variation
between parents mainly in inbreeding species.
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AFLP
Amplified Fragment Length Polymorphism; a
molecular marker generated by a combination
of restriction digestion and PCR amplification.
The power of this procedure is that you can
generate a large number of map able loci with
a single amplification.
This will help you saturate a region of the
genome rather quickly.
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Thus marker allows the simultaneously
screening of a large number of anonymous
markers randomly distributed throughout the
genome.
The drawback is that procedure is a bit time
consuming.
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Sequence Tagged Sites
STS is simply a short DNA sequence generally
100 to 500 bp and occurs only once in the
chromosome or genome.
STS mapping is performed by multiple STS or
set of STS on broken/fragmented
chromosome/genome.
A collection of DNA fragments is made by
isolating a chromosome and then breaking it
into smaller pieces, so that in collection a single
point can be represented about five/six times.
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The mapping is performed by amplification of
STS unique sequence using PCR and looking
for the presence of two different STS on the
same fragment from the collection.
The frequency of having two STS on the same
fragment depends how close they are to each
other.
Closer the STS to each other higher the chance
to find them together on the more fragments ,Or
frequency at which breaks occur between two
markers.
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Any unique DNA sequence can be
used as an STS -
The STS can be any sequence which:
• Have known sequence
• Should have unique position in
chromosome/genome
The most common STS are:
• Expressed sequence tags (ESTs) (taken from
cDNA projects: limited to genes only)
• Simple sequence length polymorphism
(SSLPs) (mini and micro satellite )
• Random genomic sequences
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Comparison between markers
used in mapping
features RAPD AFLP STS
Efforts to generate
marker
Simple Simpler than
RFLP
Difficult
Reproducibility Moderate High high
Dominance Dominant Co dominant Co dominant
Information
generated
High Very high Very high
Time required for
detection
Short Longer than other short
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Importance of gene mapping
Gene map is the anatomy of genome. It is a prerequisite to understand functioning of genome.
Helps in analysis of the heterogeneity and segregation of genetic diseases.
Helps to develop methods for gene therapy.
Provides clinically useful information about linkage.
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QUERY????? (IF ANY)
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